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通过Ccr-Emd组合驱动的丁酰辅酶A形成途径从葡萄糖生物合成聚(3-羟基丁酸酯-3-羟基己酸酯)

Biosynthesis of Poly(3-hydroxybutyrate--3-hydroxyhexanoate) From Glucose by Through Butyryl-CoA Formation Driven by Ccr-Emd Combination.

作者信息

Saito Shu, Imai Ryu, Miyahara Yuki, Nakagawa Mari, Orita Izumi, Tsuge Takeharu, Fukui Toshiaki

机构信息

School of Life Science and Technology, Tokyo Institute of Technology, Yokohama, Japan.

School of Materials and Chemical Technology, Tokyo Institute of Technology, Yokohama, Japan.

出版信息

Front Bioeng Biotechnol. 2022 May 12;10:888973. doi: 10.3389/fbioe.2022.888973. eCollection 2022.

Abstract

Poly[()-3-hydroxybutyrate--()-3-hydroxyhexanoate] [P(3HB--3HHx)] is a practical kind of bacterial polyhydroxyalkanoates (PHAs). A previous study has established an artificial pathway for the biosynthesis of P(3HB--3HHx) from structurally unrelated sugars in , in which crotonyl-CoA carboxylase/reductase (Ccr) and ethylmalonyl-CoA decarboxylase (Emd) are a key combination for generation of butyryl-CoA and the following chain elongation. This study focused on the installation of the artificial pathway into . The recombinant strain of JM109 harboring 11 heterologous genes including Ccr and Emd produced P(3HB--3HHx) composed of 14 mol% 3HHx with 41 wt% of dry cellular weight from glucose. Further investigations revealed that the C monomer ()-3HHx-CoA was not supplied by ()-specific reduction of 3-oxohexanoyl-CoA but by ()-specific hydration of 2-hexenoyl-CoA formed through reverse β-oxidation after the elongation from C to C. While contribution of the reverse β-oxidation to the conversion of the C intermediates was very limited, crotonyl-CoA, a precursor of butyryl-CoA, was generated by dehydration of ()-3HB-CoA. Several modifications previously reported for enhancement of bioproduction in were examined for the copolyester synthesis. Elimination of the global regulator Cra or PdhR as well as the block of acetate formation resulted in poor PHA synthesis. The strain lacking RNase G accumulated more PHA but with almost no 3HHx unit. Introduction of the phosphite oxidation system for regeneration of NADPH led to copolyester synthesis with the higher cellular content and higher 3HHx composition by two-stage cultivation with phosphite than those in the absence of phosphite.

摘要

聚[(R)-3-羟基丁酸酯-共-(R)-3-羟基己酸酯][P(3HB-共-3HHx)]是一种实用的细菌聚羟基脂肪酸酯(PHA)。先前的一项研究已经建立了一条从结构不相关的糖类生物合成P(3HB-共-3HHx)的人工途径,其中巴豆酰辅酶A羧化酶/还原酶(Ccr)和乙基丙二酰辅酶A脱羧酶(Emd)是生成丁酰辅酶A以及后续链延伸的关键组合。本研究着重于将该人工途径导入[具体对象未提及]。携带包括Ccr和Emd在内的11个异源基因重组的JM109菌株,以葡萄糖为原料产生了由14摩尔% 3HHx组成的P(3HB-共-3HHx),占干细胞重量的41%。进一步研究表明,C单体(R)-3HHx-CoA不是由3-氧代己酰辅酶A的(R)-特异性还原提供的,而是由从C到C链延伸后通过逆向β-氧化形成的2-己烯酰辅酶A的(R)-特异性水合作用提供的。虽然逆向β-氧化对C中间体转化的贡献非常有限,但丁酰辅酶A的前体巴豆酰辅酶A是由(R)-3HB-CoA脱水产生的。为了提高共聚酯的合成效率,研究了先前报道的几种用于提高[具体对象未提及]生物合成的修饰方法。去除全局调节因子Cra或PdhR以及阻断乙酸盐的形成会导致PHA合成不佳。缺乏核糖核酸酶G的菌株积累了更多的PHA,但几乎没有3HHx单元。引入用于NADPH再生的亚磷酸氧化系统,通过亚磷酸两阶段培养,导致共聚酯合成具有比不存在亚磷酸时更高的细胞含量和更高的3HHx组成。

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